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A rat genetic map constructed by representational difference analysis markers with suitability for large-scale typing.

机译:通过具有代表性的差异分析标记构建的大鼠遗传图谱适合大规模打字。

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摘要

Representational difference analysis (RDA) was applied to isolate chromosomal markers in the rat. Four series of RDA [restriction enzymes, BamHI and HindIII; subtraction of ACI/N (ACI) amplicon from BUF/Nac (BUF) amplicon and vice versa] yielded 131 polymorphic markers; 125 of these markers were mapped to all chromosomes except for chromosome X. This was done by using a mapping panel of 105 ACI x BUF F2 rats. To complement the relative paucity of chromosomal markers in the rat, genetically directed RDA, which allows isolation of polymorphic markers in the specific chromosomal region, was performed. By changing the F2 driver-DNA allele frequency around the region, four markers were isolated from the D1Ncc1 locus. Twenty-five of 27 RDA markers were informative regarding the dot blot analysis of amplicons, hybridizing only with tester amplicons. Dot blot analysis at a high density per unit of area made it possible to process a large number of samples. Quantitative trait loci can now be mapped in the rat genome by processing a large number of samples with RDA markers and then by isolating markers close to the loci of interest by genetically directed RDA.
机译:应用代表性差异分析(RDA)分离大鼠中的染色体标记。四个系列的RDA [限制酶,BamHI和HindIII;从BUF / Nac(BUF)扩增子中减去ACI / N(ACI)扩增子,反之亦然]产生131个多态性标记;将这些标记中的125个映射到除X染色体之外的所有染色体。这是通过使用105只ACI x BUF F2大鼠的作图面板完成的。为了补充大鼠中染色体标志物的相对缺乏,进行了遗传指导的RDA,其允许分离特定染色体区域中的多态性标志物。通过改变该区域附近的F2驱动程序-DNA等位基因频率,从D1Ncc1基因座分离了四个标记。 27个RDA标记中的25个提供了​​有关扩增子的斑点印迹分析的信息,仅与测试扩增子杂交。高密度每单位面积的斑点印迹分析使处理大量样品成为可能。现在可以通过使用RDA标记处理大量样品,然后通过遗传定向RDA分离接近目标基因座的标记,在大鼠基因组中定位定量性状基因座。

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